Clinical impact of chromosomal aberrations in patients
with Multiple Myeloma
Luba Trakhtenbrot , Galina Ishoev and Ninette Amariglio Hematology Laboratory, The Chaim Sheba Medical Center, Tel-Hashomer
“Chromosome analysis is currently the most important tool to assess
risk and predict outcome in MM.
With the development of new drugs in combinations with alternative
transplantation modalities or in new combinations without transplantation
– chromosome analyses will probably be even more important for
selection of the best treatment for individual patients.
Chromosome analysis should be performed in all patients with
MM.”
H. Nahi, 2010, Hematology Centre, Karolinska University
Hospital, Stockholm, Sweden
A chromosome is made of two
identical molecules of DNA
efficiently packed into sister
chromatids, which are held together
at their centromere.
Each human chromosome has a
short arm ("p" for "petit") and long
arm ("q" for "queue") separated by
a centromere.
The centromere is the structure
where the mitotic spindle attaches
prior to segregation. The ends of the
chromosome are called telomeres.
A chromosome is the visible state of genetic material
During cell division, mitosis, the chromosomes
become highly condensed and are then visible as dark distinct
bodies within the nuclei of cells.
.
G-banding
The band width and the order of bands are
characteristics of a particular chromosome
Standard G band staining techniques allow
between 400 and 600 bands to be seen on metaphase chromosomes
Preparation of mitotic chromosomes
Min – 5 days
Max - 3 months
blood/BM
Structural Chromosomal rearrangements
Inversions
Duplication
s
Deletions
Translocations t(9;14;2
2)
t(6;9)
Ploidy level: The diploid number ( n = 46) is the number of chromosomes of a normal cell.
Hyperdiploid – 47-57; Hypodiploid – 35-45 chromosomes
Triploid = 3n = 72; near triploid – 58 – 80 chromosomes;
Tetraploid = 4n = 96 ; near tetraploid – 81 – 103 chromosomes
Numerical abnormalities: the loss of chromosome(s) and the gain of chromosome(s)
Chromosome rearrangements in hematological cancer diseases No. of rearrangements ~ 540 / No. of cloned breakpoints ~350 / No. of genes involved 90
Clinical applications:
Diagnosis
CML = BCR/ABL fusion =
t(9;22)(q34;q11)
APL = RARA rearrangements =
t(15;17)(q24;q21) and other
translocations with 17q21
Prognostic factor
Independent predictor of outcome in
MDS, AML, MF and ALL
Marker
for the detection of the minimal residual
disease (MRD)
Low rate of proliferation of the plasma cells (PCs) and
a low percentage of PCs in bone marrow samples
Conventional karyotype analysis is informative
in only 30% of MM cases
Chromosomal abnormalities (translocations , gains and losses )
are very frequent in myeloma:
most MMs show an average of 11 abnormalities per karyotype.
.
M-FISH
1.46,XY,der(1)t(1;4)(p12;p12)dup(1)(q25q32),+dup(5)(q13q31),+der(1;7)(p10;q10),der(8)t(4;8)(q31
;p23),+del(9)(q22),der(11)t(11;13)
(p15;q14),+14,+15,16,der(20)t(1;20)(p13;p11),der(21;22)(q10;q10)[cp17]/46,XY[29]
2. 47–52,X,der(X)t(X;1)(q28;q25),der(1)t(1;21)(q44;q11),+del(1)(p13),+3,+5,+7,+11,+15,
der(16)t(16;17)(q24;q21),+19,–20[cp5]/46,XX[38]
3. 45,X,–X,der(2)t(2;2)(p21;q21),del(3)(q13),del(3)(q25),add(4)(p12),del(5)(p12), 74
psu dic(5;1)(q35;q10),del(6)(q21),del(11)(q23),t(11;14)(q23;q32),del(12)(q12q14),+12,–
13[cp12]/46,XX[18]
4. 44–45,XX,del(6)(q21q23),der(10)t(10;10)(p15;q11),–9,–11,–12,der(14)t(2;14) 16.4
(p13;q32),+del(21)(q22),+r[cp6]/46,XX[7]
5. 41–43,X,–Y, der(1;15)(q10;p11)ins(1)(q32;q12),+del(1)(p13),t(4;20)(p15.2;p13), 55.9del(5)(p13),–
7,–8,del(10)(p12.2),–13,–
14,t(14;16)(q32;q23),der(16)t(16;17)(q12;q21),+21,del(22)(q11.2),+mar[cp34]/46,XY[3]
The complexity of structural and numerical chromosomal aberrations
typical for MM has made it difficult to determine the individual
prognostic contribution of specific chromosomal alterations.
The most common chromosomal abnormalities in MM
detected by conventional cytogenetics
Structural abnormalities:
Rearrangements involving 14q32 (IGH gene) with various partner genes -
translocations t(4;14); t(11;14); t(14;16), t(14;20) and other (70%)
Chromosome 13 deletions and monosomy(>50% )
Deletion of chromosome 17p (p53 gene)
Chromosome 8q24 rearrangements (c-myc gene)
Ploidy alterations:
Hypodiploidy and Hyperdiploidy > 50%
In clinical practice, the optimal method to detect chromosomal
aberrations and ploidy in MM is interphase fluorescence in situ
hybridization (I-FISH)
FISH is the technique in which a DNA
probe is labeled with a fluorescent dye
(that can be visualized under a
fluorescent microscope) and then
hybridized with target DNA on a
microscopic slide.
When DNA is heated, DNA strands
break apart, or denature, and the probes
are able to hybridize to their
complementary sequence in target
DNA.
I-FISH is used to enumerate
chromosomes and to detect
chromosomal deletions, translocations,
or gene amplifications in cancer cells.
Interphase FISH
Metaphase FISH
Normal status
FISH detection of 13q and 17p deletions
Control probe 13q or 17p probes
Deletion Monosomy
3’ to centromere 5’ Telomere
Detection of the 14q32 alterations by the
IGH gene Break Apart Rearrangement Probe
#14
#14
#14
der14 der??
Detection of the translocations t(4;14), t(6;14),
t(11;14) , t(14;16) and t(14;20)
Normal
#14 #14
#4/11/16
#4/11/16
#14 #4/11/16
der 14
der4/11/16
Translocation
14 14 4/11/16 der14 der4/
11/16
Green labeled I GH segment
Red labeled segments
of chromosomes 4/6/11/16/20
Fusion between IGH and
chromosomes 4/11/16
1 2
t(11;14) /11q A
Y/O/G Y/O/G2
#11 #14
der 14
der 11
#14
der 11
der 14
G2Y/O/ Y/O/G
t(11;14) /11q B
4
5
7
t(11;14),del Var IgH
on #14 /11q A
3
#11 #14
der 14
Y/O/G2 der 11
O/G2
#14
der 11
der 14
8
#11 #14
der 14
der 11
#14
der 11
IGH/CCND1 IGH
IGH/CCND1 IGH
der 14
Y/O/G/small G
#11 #14
der 14
der 11
#14
der 11
t(11;14); partial del Var
IgH on der11/11qB
Y/O/G
der 14
t(11;14); 2x del IgH Var
on #14/ 11qA
#14
O/G3 G2Y/O/2
#14 #11
der 14
der 11
der 14 #14
der 11
#14
O/G2Y/
t(11;14); del Var IgH
on der11/11qA
Y/O
der 14
#14 #11
der 14
der 11
#14
6 O/G2Y/
#11
der 14
der 11
#14
der 11
Y/G
t(11;14); del Const IgH on
der14/11qA
G2Y/O/ O/G2
#11 #14
der 14
der 11
#14
der 11
t(11;14), del Var IgH on
#14 /11q B
der 14
11
9
10
12
13
15
t(11;14),+der14/ 11qA
#14 #11
der 11
der 14 der 14
Y/O/G3
der 14
O/G2Y/
#14
der 11
der 14
Y/O/G2
t(11;14); +#14/ 11qA der 14
#14
der 11
#14
16
#14
der 14
IGH/CCND1 IGH IGH/CCND1
IGH
Y/O/G
der 14
der 11
14
der 14
der 11
#11
t(11;14); - #14/11qB
O/G
#14 #11
der 11 der 11 Y/O/G Y/G
#14
t(11;14); - der14/11qA
t(11;14); - #14/11qA
Y/O2 O/G
der 11
#11
der 14 der 14
der 11
t(11;14); - der11
Y/O/G Y/O
#11
der 14
#14
der 14
#14
der 14
der 11 G2Y/O/2
#11 #14 #14
Typical t(11;14);++#11,-der11
#14
der 14
Y/O O/G3Y/
#11 #11
#11
O/G3Y/
t(11;14),++der14/ 11qA
der 14
der 14 #14 #11
der 11 Y/O/4
G
der 14 #14 der 14
der 11
der 14
der 14
A high heterogeneity of translocation t(11;14)
that was overlooked in previous investigations.
FISH - high false positive rates ( 1-10%)
There are major problems with the quality of the bone marrow aspirates received for
FISH studies; these frequently contain drastically fewer PCs than the corresponding
smear used for morphological assessment.
It is difficult for clinicians to accept that a normal FISH result from a patient that had
80% PC on the morphology slide could be meaningless, but that is the reality.
Clinicians should be encouraged to send part of the first draw of the aspirate for FISH
studies ! [Ross F. et al., 2012]
The median proportion of plasma cells, is commonly low, ranging from 1-20%,
within the bone marrow aspirates.
The FISH technique cannot be performed directly as in other
hematologic malignancies PCs need to be selected, either
by flow cytometry or immunomagnetic-bead based PC sorting
(CD-138+ purified PCs)
by the concomitant labeling of the cytoplasmic immunoglobulin light chain
by image analysis systems allowing morphological assessment of PCs and FISH
scoring only in those designated as PC
All of these methods give good results ,the choice should be left to individual laboratories
A significant fraction of samples will have too few PCs to allow such analyses to be
made and will censor some patients in subsequent clinical evaluation.
Report from the European Myeloma Network on interphase FISH
in multiple myeloma and related disorders Fiona M. Ross,1 Hervé Avet-Loiseau,2 et al, 26 European Medical Centers
May-Grünwald –Giemsa staining
Sample
Processing
Cytospin
FISH
The system is capable of performing high resolution,
full color, automated or interactive morphological
and fluorescent scanning
It saves the coordinates and images of all cells found
on the slides for future reference during the next
phases of analysis
It classifies the cells according their morphology
after MGG staining into six classifications:
lymphocytes, PMN, normoblasts, myelocytes, blasts
and PC.
Detection of the chromosome 13q status in the BM cells of patients
with multiple myeloma (MM)
13q-
FISH False positive rates =8-12%
Concentration of plasma cells in bone marrow = 1-30%
del(13q)
PC
The use of the combined
morphological and FISH analysis
enables the most precise
determination of chromosome 13
status in new diagnosed and treated
MM patients [Hardan et al., Exp.
Hematology 32 (2004)]
2011-2013 – combined morphological and FISH analysis
of 25-40 cases /month
Deletion and
subsequent
tetraploidisation
(duplication of the
hybridization pattern)
Normal pattern with
two 13q signals
X2
Tetraploidisation del 13q
Abnormal pattern
with
one 13q signal
Chromosomal abnormalities are associated with prognosis in MM:
The detection of t(4;14), t(14;16), deletions of chromosome 13 and p53 will
define high-risk prognostic groups that are not generally controlled with high-
dose melphalan and autologous stem cell transplantation (ASCT), and should
therefore be treated with more investigational therapies.
Alternatively, eligible patients who do not have these poor risk factors are more
likely to benefit from a high-dose, melphalan-based, regimen followed by ASCT.
Patients with t(11;14) were initially believed to have an unfavorable category of
MM, but in recent works their improved outcome was confirmed.
Non-hyperdiploidy is also proposed as an adverse prognostic factor
Neutral prognosis t(11;14), t(6;14)
Hyperdiploidy
Poor prognosis
t(4;14); IGH@-FGFR3
t(14;16); IGH@-MAF
t(14;20); IGH@- MAFB
P53 deletion
Gain of 1q /Deletion of 1p
16q deletion
However, in the study of patients with relapsed or refractory MM who received
treatment with lenalidomide plus dexamethasone, del(13g) was associated with a
lower overall response rate (ORR) and a shorter progression-free survival (PFS).
Was suggested that prognostic value of del(13q) may be different at diagnostic and
later stages of the disease. [Avet-Loiseau H. et al., 2010]
Prognostic significance of del13q detected by FISH
Conflicting results!
In early investigations it was recognize as prognostic marker independent on the
mode of treatment [Fonseca R. et al.,2004; Leibish P, 2006].
However, was shown that isolated del(13q) ( it means , without t(4;14) or
del17p), is not associated with a poor prognosis, thus prognostic value of del13q
may be related to prognostic impact of associated other poor-risk markers
[Chiecchio L. et al., 2009, Fonseca R. et al., 2009].
Prognostic significance of 1q+/1p- detected by FISH
Conflicting results!
Chromosome 1 abnormalities, particularly 1q gain(s) and 1p loss are a frequent
finding in MM that are associated with disease progression ( transition from
MGUS/SMM to MM) , shorter progression-free survival (PFS) and overall survival
(OS). 1q2+ was identified as an independent factor predicting OS in the context of
treatment with lenalidomide and dexamethasone in patients with recurrent MM
[Chang H. et al., 2010.2011; Klein U. et al., 2011]
However, later was shown that 1q21 gains with additional genetic abnormalities
but not isolated 1q21 gain is a negative prognostic factor in newly diagnosed
patients with multiple myeloma treated with thalidomide-based regimens
[Grzasko N et al., 2012]
Combination of translocations with numerical aberrations The presence of trisomies in patients with t(4;14), t(14;16), t(14;20) or p53 deletion
ameliorates the usual adverse impact associated with these prognostic markers. Mayo Clinic. Rochester, MN; Mayo Clinic in Arizona, Scottsdale, AZ, USA, 2012
t(14;16)
t(14;20)
t(11;14)
t(4;14)
Other
IGH rearr
t(4;14)
t(11;14)
No IGH
rearr
Other IGH
rearr
No IGH
rearr
13q norm del 13q
The proportion of IGH abnormalities in the del13q group is
three time higher than in the 13q norm group (~ 1000 cases)
Two major genetic categories of MM according to ploidy status: [Smadja N,et al., 1998; Fonseca R, et al.,2003]
The nonhyperdiploid MM (< 48 chromosomes or more than 74
chromosomes) : associated with primary translocations such as t(11;14),
t(4;14), and t(14;16) = Abnormal IGH
The hyperdiploid MM (48 to 74 chromosomes, median 53 chromosomes):
associated with trisomies especially of chromosomes 3, 7, 9, 11, 15, and 19.
No /less)translocations evolving IGH
Using the criteria of 2 or more trisomies from a 3-chromosome combination
(+9,+ 11,+ 15), hyperdiploid myeloma can be detected with high specificity
Normal IGH
FISH with t(11;14) probe:
Detection of rear types of t(11;14) (~3% of all the t(11;14)
Detection of +11 = the possibility of hyperdiploidy
Normal IGH = hyperdiploid MM?
27.6%
del 13q 13q norm
1q+/1p-
p53-
49.0% 13.4%
0.6%
0
20
40
60
80
100
120
140
160
180
200
1 2 3 4 del
13q
13q
norm
P53-
1q21+
Normal
p53 and
1q21
Proportion of cases with p53- and 1q+/1p-
significantly higher in del 13q group
Normal IGH
del p53
1q+/1p-
13q norm
IGH norm
IGH norm
del 13q
Hyperdiploidy
1q+/1p-
Proportion of cases with high-risk translocations
t(4;14), t(14;16) and t(14;20)
is significantly higher in the 13q-group
t(4;14)
t(11;14)
t(14;16) t(14;20)
t(11;14)
t(6;14)
del 13q 13q norm
t(4;14)
t(11;14)
No IGH
rearr
Other IGH
rearr
13q norm del 13q
t(6;14)
t(14;16)
t(14;20)
No IGH
rearr
Other
IGH rearr t(11;14)
t(4;14)
Abnormal IGH
0
20
40
60
80
100
120
1 2 3 4
1סידרה
2סידרה
3סידרה
t(14;16)
t(4;14)
t(11;14)
16q- 1q+/1p- p53- del 13q-
In t(14;16) and t(4;14) groups:
proportion of 13q- and 1q+/1p- is significantly higher than in t(11;14);
proportion of p53- and 16q- is almost the same
Aberrations of P53 gene are the most predictive molecular markers for resistance to
therapy and short overall survival (OS).
The prognosis for the group of MM patients with P53- is clearly worse than the
prognosis for patients with any of the other established unfavorable chromosomal
abnormalities, regardless of therapy including allogeneic transplantation.
Unknown IGH rearrangements Proportion of cases with p53- and 1q+/1p-
is high in both groups – 13q norm and del13q-
del 13q 13q norm
1q+/1p-
p53-
58% 30%
7% 13%
13q norm
Unknown
IGH rearr
Del 13q
Unknown
IGH rearr
del p53
1q+/1p-
16q- ?
del(13q)
del(IGH)
del(17p)
1p loss
plusqqq
del(16q)
1q gain
.6.7.8.91matching similarity measure
complete linkage, matching measure - 11_14
Translocation t(11;14)
del 1p , del p53 and 1q gains are very mutually similar (Y ≥0.9) and
has a strong association with del(16q) (Y = 0.80) and 1q gain(Y ~0.73).
del (IGH) and del(13q) are very mutually similar (Y ~ 0.87);
Also this couple has also association with others (Y~0.60).
All of the chromosome aberrations are associated
1q gain
del 13q
del IGH
del 1p
del p53
1q gains
del(16q)
t(11;14)
Hyperdiploidy 13q norm
IGH norm
13q norm
IGH rearr
del 13q
IGH rearr
del 13q
IGH norm
del p53
1q+/1p-
16q- ?
t(4;14)
t(14;16)
t(14;20)
t(11;14)
“Wherever possible, testing should carried out
for t(4;14)(p16;q32), t(14;16)(q32;q23), p53
deletions, 1q gains (and 1p deletions in
patients suitable for autograft).
An extended panel may include testing for
t(11;14)(q13;q32), t(14;20)(q32;q12), ploidy
status, and chromosomes12 and 13
abnormalities.”
Report from the European
Myeloma Network on
interphase FISH in multiple
myeloma and related disorders Fiona M. Ross,1 Hervé Avet-Loiseau,2 et
al, 26 European Medical Centers
Galina Ishoev and Bella Weisman
THANK YOU VERY MUCH!!